PLASMID MINI-PREP KIT - Column Type

ORDERING INFORMATION

Catalog #	Product	Amount	Price (EUR)
# PLA 50	ROVALAB Plasmid Mini-Prep Kit	50 preparations	43,50
# PLA 250	ROVALAB Plasmid Mini-Prep Kit	250 preparations	176,50

PRODUCT COMPONENTS

Buffer	# PLA 50	# PLA 250
Resuspension Buffer	16 ml	80 ml
RNase A	2 mg	5 x 2 mg
Lysis Buffer	16 ml	80 ml
Neutralization Buffer	20 ml	100 ml
Column Activation Solution	6 ml	30 ml
Elution Buffer	6 ml	30 ml
Spin Columns & 2ml Tubes	50	250

DESCRIPTION

ROVALAB Plasmid Mini-Prep Kit is designed for isolation of high-purity plasmid or cosmid DNA from cells for subsequent sequencing, restriction digests, or transformations. The 2-step alkaline lysis procedure and spin column based preparation provide a fast, easy and efficient way of DNA isolation without shearing or significant loss of product. It allows elution in a small volume of low-salt buffer. Time-consuming phenolchloroform extraction or alcohol precipitation is eliminated. The kit can be used either in micro-centrifuges or on vacuum manifolds and allows the extraction of up to 20 µg DNA per preparation.

FEATURES

• Spin column type
• Binding capacity: 20 µg DNA/column
  
• Quick mini prep of pure plasmid
  
• Sequencing & transfection grade
• Low copy plasmid, large size circular DNA (formid, BAC clones) prep
  

APPLICATIONS

• General sequencing
• Transfection
  
• Cloning

BASIC PROTOCOL

The DNA purification follows a simple binding, washing and eluting procedure. The optional secondary washing step minimizes the salt content of the purification product.

Before start, prepare the following components:

• Add total RNase A to the Resuspension Buffer and mix well. RNase A containing Resuspension Buffer should be stored at 4°C.
• for 50 preparations (# PLA 50): add 2 mg RNase A to 16 ml Resuspension Buffer
• for 250 preparations (# PLA 250): add 5 x 2 mg RNase A to 80 ml Resuspension Buffer
• Prepare an 80% Ethanol (V/V) solution as Washing buffer. Please note that the Ethanol concentration of Washing Buffer may decrease during long time storage resulting in a possible drop of the final DNA yield.
• for 50 preparations (# PLA 50): 80 ml
• for 250 preparations (# PLA 250): 400 ml

1. Cell Harvest and Suspension

• Harvest the bacterial cell culture (1-3 ml) by centrifugation.
• Resuspend pelleted bacterial cells in 300 μl Resuspension Buffer containing RNase A by pipetting. 

2. Cell Lysis and Neutralization

• Add 250 µl Lysis Buffer and mix gently by inverting the tube 4-6 times (do not vortex!).
• Add 350 µl of Neutralization Buffer and invert immediately 4-6 times.
• Centrifuge at 12,000 g for 10 min at room temperature in a microcentrifuge.

3. Column Activation

• Place a Spin Column into a 2 ml collection tube.
• Add 100 µl of Column Activation Solution into the Spin Column.
• Centrifuge at 12,000 g for 30 sec in a microcentrifuge.
  

4. Column Loading

• Apply the supernatant from step 2 into the activated Spin Column by decanting or pipetting.
• Centrifuge at 12,000 g for 30 sec in a microcentrifuge.
• Discard the flow-through.

5. Column Washing

• Place the DNA loaded Spin Column into the used 2 ml tube.
• Apply 700 µl of Washing Buffer (80% Ethanol) to the Spin Column.
  
• Centrifuge at 12,000 g for 30 sec and discard the flow-through.
  
• Optional Secondary Washing: Recommended only for DNA >200 bp, if highly purified DNA (for DNA sequencing, transfection etc.) is required.
• Add 700 µl of Washing Buffer to the Spin Column.
• Centrifuge at 12,000 g for 30 sec and discard the flow-through.
• Centrifuge again for 2 min to remove residual Washing Buffer.

6. Elution

• Place the Spin Column into a clean 1.5 ml microtube (not provided in the kit).
• Add 30-50 μl Elution Buffer to the center of the column membrane.
• Incubate at room temperature for 1 min.
• Centrifuge at 12,000 g for 1 min to elute DNA.
  

STORAGE

Store at room temperature (15 – 25 °C) for 12 months.

For long term storage place RNase A lyophilisate at -20°C.

RNase A containing Resuspension Buffer should be stored at 4°C.